Characterization of Aspergillus niger Pectate Lyase A,

Abstract

The Aspergillus niger plyA gene encoding pectate lyase A (EC 4.2.99.3) was cloned from a chromosomal λ_EMBL4 library using the Aspergillus nidulans pectate lyase encoding gene [Dean, R. A., and Timberlake, W. E. (1989) Plant Cell 1, 275−284] as a probe. The plyA gene was overexpressed using a promoter fusion with the A. niger pyruvate kinase promoter. Purification of the recombinant pectate lyase A resulted in the identification of two enzyme forms of which one appeared to be N-glycosylated and the other appeared to be free of N-glycosylation. The two enzyme forms showed identical specific activities. The N-glycosylation free pectate lyase A was further characterized with respect to product formation on polygalacturonic acid (α-1,4 linked d-galacturonic acid) and mode of action on oligogalacturonides of degree of polymerization 2−8. The bond cleavage frequencies for tetra-, penta-, and hexagalacturonides were studied as a function of [CaCl₂]. The bond cleavage frequencies changed in a [CaCl₂]-dependent way for penta- and hexagalacturonide. Kinetic studies using tetra- and hexagalacturonide revealed a strong sigmoidal [CaCl₂]-dependent relation. The role of Ca²⁺ ions in substrate binding is discussed.